精子介导GFP基因在小鼠早期胚胎中的表达

利用 DIG 末端标记技术和免疫组化技术分析了小鼠精子体外结合内化外源DNA的效率。试验结果表明,不同小鼠个体的精子结合外源DNA的阳性率有明显差异（P<0.01）,平均为13%。利用考马斯亮蓝染色评价了小鼠精子顶体反应发生的情况,筛选出TYH培养液为较合适的体外受精液。利用小鼠体外受精技术,将体外转染GFP基因并获能的小鼠精子与成熟卵母细胞进行体外受精,受精卵进行体外培养,表达GFP胎的阳性率为4.7%。验证了精子介导制备转基因小鼠胚胎的可行性,并建立了利用精子载体法制备转基因小鼠胚胎的平台。     

精子介导GFP基因在小鼠早期胚胎中的表达

利用DIG末端标记技术和免疫组化技术分析了小鼠精子体外结合内化外源DNA的效率。试验结果表明,不同小鼠个体的精子结合外源DNA的阳性率有明显差异(P<0.01),平均为13%。利用考马斯亮蓝染色评价了小鼠精子顶体反应发生的情况,筛选出TYH培养液为较合适的体外受精液。利用小鼠体外受精技术,将体外转染GFP基因并获能的小鼠精子与成熟卵母细胞进行体外受精,受精卵进行体外培养,表达GFP胚胎的阳性率为4.7%。验证了精子介导制备转基因小鼠胚胎的可行性,并建立了利用精子载体法制备转基因小鼠胚胎的平台。     

哺乳动物早期胚胎的基因表达及其调控

哺乳动物的早期发育包括合子的形成、胚胎基因组的活化和细胞开始分化等。在这段时期,精蛋白被组蛋白取代;二倍体形成后甲基化的单倍体亲本基因组经历了脱甲基作用;母本控制的发育被合子控制所取代。此外,在染色体调节的转录抑制状态形成之后,胚胎基因组活化,但基因的有效表达需要有增强子。这种转录抑制状态的产生很可能发生在染色质结构水平,因为诱导组蛋白过乙酰化可免除对增强子的需求。早期胚胎的mRNA表达模式与在体内或体外成功发育的关系,对确定最佳培养条件和核移植程序是必不可少的。     

重组腺病毒介导VEGF121 cDNA体外转移与表达

构建携带VEGF12 1cDNA重组复制缺陷型腺病毒表达载体 ,制备重组腺病毒 ,该腺病毒能介导VEGF12 1cDNA基因促进人脐静脉血管内皮细胞增殖 ,促进毛细血管管腔样结构形成 .ELISA检测表明VEGF12 1cDNA基因表达产物分泌至培液上清 ,并显示强烈血管通透作用 .为进一步利用重组腺病毒介导VEGF12 1cDNA进行缺血性疾病的基因治疗奠定良好的基础     

Diet Composition and Lipids of In Vitro-Produced Heterorhabditis bacteriophora

Several entomopathogenic nematode species are currently under evaluation for mass production and field efficacy for biological control of insect pests. However, quality and quantity of in vitro-produced entomopathogenic nematodes vary considerably, depending on media, temperature, and production method. In addition, nematode production should be cost effective. We investigated nematode yield, production time, total lipid content, and fatty acid composition of Heterorhabditis bacteriophora produced in artificial media supplemented with different lipid sources. Lipid source significantly affected lipid quantity and quality in H. bacteriophora. Media supplemented with extractable insect lipids produced yields 1.9 times higher than did beef fat- or lard-supplemented media. Moreover, the developmental rate in media supplemented with host lipids was 1.7 times faster than that in media supplemented with beef fat or lard. Nematodes grown in media supplemented with insect lipids accumulated significantly higher lipid proportion per dry biomass than those grown in media supplemented with other lipid sources. H. bacteriophora produced in media supplemented with insect lipids, olive oil, or canola oil had similar fatty acid patterns, with oleic (18:1) acid as the major lipid fatty acid. Media supplemented with other lipid sources produced nematodes with fatty acid patterns different from those of media supplemented with insect lipids. We recommend addition of fatty acid mixtures that resemble natural host lipids for mass-producing entomopathogenic nematodes. This could provide nematode quality similar to in vivo-produced nematodes and could improve yield.     

电穿孔技术在转基因及动物克隆中的应用

电穿孔技术利用电场造成细胞膜的改变而将DNA导入细胞内,它还可用于细胞融合及动物克隆等。基因电转移的效率通常比化学法提高1—2个数量级,主要与脉冲波形、长度、缓冲液等有关。方波直流电脉冲应用广泛,在有关细胞核移植的多项研究报告中均指出它有重要作用。     

牛FABGL基因的克隆及其与牛生物经济学性状的相关分析

运用同源序列克隆技术结合反转录PCR技术和3′,5′cDNA末端快速扩增技术得到了牛FABGL基因的完整CDS,3′非翻译区和部分5′非翻译区.序列分析和生物信息学研究表明,所获得的牛FABGL基因的cDNA包含994个核苷酸和780 bp的开放阅读框及198 bp的完整的3′非翻译区.该基因编码260个氨基酸残基蛋白,在氨基酸水平上与人的同源基因具有高度的相似性(88%).采用PCR-SSCP方法,在递交的包含完整CDS的长为1 925 bp的该基因的基因组DNA序列(GenBank接受号DQ409814)1 065 bp 和1 792 bp处,分别发现了两个单核苷酸碱基突变Y=C/T,R=A/G;它们分别位于该基因的第五和第八内含子.对包含这两个多态位点的3个品种(安格斯、海福特和西门塔尔)牛的共179个个体等位基因频率与部分肉质及生长性状进行了关联分析,结果发现,在第八内含子内具有GG基因型的个体的肉用性能指数(4.283±.0.475kg/cm)较具有AA基因型个体的(4.008±0.465kg/cm)高(P≤0.01);而且同一位点具有GG基因型的个体的眼肌面积(73.380±13.005 cm2)显著高于具有AA基因型的个体(67.744±12.777 cm2)(P≤0.05).在第五内含子内,具有CC、CT、TT3种不同基因型的个体之间,平均日增重差异均达到极显著水平(P≤0.01),以具有TT基因型的个体平均日增重最高(0.652±0.330kg/d),CC基因型的最低(0.421±0.178kg/d).     

牛组织中MBD1基因表达及其DNA甲基化调节

DNA甲基化是主要的表观遗传调节方式,在转录水平调节基因的表达,甲基化CpG结合蛋白MBD1能够结合甲基化及非甲基化的DNA,通过抑制域抑制基因的转录,在DNA甲基化和转录抑制之间起重要作用,但DNA甲基化对MBD1自身的调节作用还不清楚.本研究首先利用RT-PCR检测成年牛心脏、肾脏、肝脏、睾丸及卵巢5种组织中MBD1基因mRNA的表达;并根据牛MBD1调节区序列,针对其中的12个CpG位点设计引物,利用甲基化PCR测序分析方法,分析该调节区的DNA甲基化状态在牛5种组织中的变化.结果表明,在牛的5种组织中,MBD1基因在心脏和肾脏的表达量低于肝脏、睾丸及卵巢,且差异显著(P＜0.05);DNA甲基化检测显示,心脏和肾脏MBD1调节区的甲基化比率较肝脏、睾丸及卵巢甲基化低,说明调控区DNA甲基化与MBD1基因的组织特异性表达相关.     

奶牛γ干扰素基因的高效表达及活性测定

经刀豆素(conA)刺激诱导奶牛外周血淋巴细胞,应用RT-PCR方法从其总RNA中对奶牛γ干扰素基因cDNA进行扩增,然后将特异性片段连接到pMD18-T载体,测序结果表明,与已知序列同源性为100%。然后将特异性片段连在pRLC载体上进行表达,经SDS-PAGE分析,原核表达产物为16kDa的重组蛋白,占菌体总蛋白的42%,表达产物以包涵体形式存在。经7mol/L盐酸胍的变性液溶解及0.5mol/L盐酸胍复性液处理,表达产物进行脱盐、凝胶层析纯化,细胞病变抑制法结果表明,重组牛IFN-γ具有较高的干扰素活性,约为6.0×105U/mg。     

奶牛γ干扰素基因的高效表达及活性测定

经刀豆素(conA)刺激诱导奶牛外周血淋巴细胞,应用RT-PCR方法从其总RNA中对奶牛γ干扰素基因cDNA进行扩增,然后将特异性片段连接到pMD18-T载体,测序结果表明,与已知序列同源性为100%.然后将特异性片段连在pRLC载体上进行表达,经SDS-PAGE分析,原核表达产物为16kDa的重组蛋白,占菌体总蛋白的42%,表达产物以包涵体形式存在.经7mol/L盐酸胍的变性液溶解及0.5mol/L盐酸胍复性液处理,表达产物进行脱盐、凝胶层析纯化,细胞病变抑制法结果表明,重组牛IFN-γ具有较高的干扰素活性,约为6.0×105U/mg.     

Cloning of the Authentic Bovine Gene Encoding Pepsinogen A and Its Expression in Microbial Cells

Bovine pepsin is the second major proteolytic activity of rennet obtained from young calves and is the main protease when it is extracted from adult animals, and it is well recognized that the proteolytic specificity of this enzyme improves the sensory properties of cheese during maturation. Pepsin is synthesized as an inactive precursor, pepsinogen, which is autocatalytically activated at the pH of calf abomasum. A cDNA coding for bovine pepsin was assembled by fusing the cDNA fragments from two different bovine expressed sequence tag libraries to synthetic DNA sequences based on the previously described N-terminal sequence of pepsinogen. The sequence of this cDNA clearly differs from the previously described partial bovine pepsinogen sequences, which actually are rabbit pepsinogen sequences. By cloning this cDNA in different vectors we produced functional bovine pepsinogen in Escherichia coli and Saccharomyces cerevisiae. The recombinant pepsinogen is activated by low pH, and the resulting mature pepsin has milk-clotting activity. Moreover, the mature enzyme generates digestion profiles with α-, β-, or κ-casein indistinguishable from those obtained with a natural pepsin preparation. The potential applications of this recombinant enzyme include cheese making and bioactive peptide production. One remarkable advantage of the recombinant enzyme for food applications is that there is no risk of transmission of bovine spongiform encephalopathy.     

p16蛋白在子宫内膜癌中表达的研究

为探讨P16基因在子宫内膜癌发生及发展过程中所起的作用,采用免疫组化SP法对38例子宫内膜癌(腺癌33例,腺棘皮癌4例,浆液性乳头状腺癌1例)及19例正常组织进行了p16蛋白的免疫组化检测,结果p16蛋白在正常组织中表达率为56.8%,在腺癌中的表达率为21.7%,在腺棘皮和浆液性乳头腺癌中的表达率为25.1%,与正常组差异显著,同时,p16蛋白在Ⅰ-Ⅱ期子宫内膜中的表达率为26.4%。而在Ⅲ-Ⅳ期子宫内膜癌中的表达率为11.7% ,二者差异显著,说明p16蛋白在子宫内膜癌的发生及进展过程中起重要作用。 Abstract:To understand the role of P16 gene in the progression of carcinoma of endometrium,the expression of P16 gene was detected in 38 carcinoma of endometrium specimens and 19 controls by immunhistochemical SP method.The p16 protein positive rates of carcinoma of endometrium and control had significant difference (P<0.05),and the expression of p16 protein was also significant different between I～II grades and III～IV grades of adenocarcinoma of endometrium.So the p16 protein was closely associated with the generation and development of the carcinoma of endometrium.     

牛β-乳球蛋白基因的克隆及其调控外源基因表达的研究

目的制备乳腺生物反应器所必需的乳腺特异性表达的调控序列,并验证其指导外源基因表达的能力.方法用PCR法从奶牛染色体上分5段扩增出了全长8.2Kb的牛β-乳球蛋白基因,包括1.8Kb的5′侧翼区、1.7Kb的3′侧翼区及4.7Kb的gDNA区.扩增出的各片段克隆到T-载体上,酶切鉴定及序列分析均证实了所扩增片段的正确性.将五个片段与荧光素酶cDNA拼接成荧光素酶瞬时表达载体并在小鼠乳腺中瞬时表达.结果注射荧光素酶瞬时表达载体的小鼠乳汁中明显测出了荧光素酶活性.结论所克隆的牛β-乳球蛋白基因表达调控序列能够指导外源基因在小鼠乳腺中表达.     

Molecular Cloning of Bovine FABGL Gene and Its Effects on Bovine Bioeconomic Traits

The complete CDS sequence of the bovine FABGL gene was determined by homology cloning approach combined with RT-PCR and 3′- and 5′-RACE. The results of sequence analysis and bioinformatics study showed that this cDNA contained 994 nucleotides, with a 780 bp open reading frame (ORF) flanked by a 16 bp 5′-UTR (incompletely) and a 198 bp 3′-UTR. The deduced amino acid sequence (260 AA) shows 88% identity with the corresponding sequence in humans. Two single nucleotide substitutions, one located in intron 5 (I5) at position 1 065 bp (Y = C/T) (GenBank: DQ409814) and the other in intron 8 (I8) at position 1 792 bp (R = A/G), were detected using the PCR-SSCP method. Analysis of the allele frequencies of the two polymorphic sites in three different cattle breeds (Angus, Hereford, and Simmental) with different genotypes showed large differences: in locus I8, cattle with the GG genotype showed higher beef performance index (BPI) (4.283 ± 0.475 kg/cm) in comparison with cattle with the AA genotype (4.008 ± 0.465 kg/cm) (P = 0.01). Regarding the ribeye area, cattle with the GG genotype showed significantly higher ribeye area (73.380 ± 13.005 cm²) compared with cattle with the AA genotype (67.744 ± 12.777 cm²) (p = 0.05). In locus I5, some associations for the average daily gain (ADG) were found at the significance level of 0.01 between three different genotypes (CC, CT, TT): cattle with the TT genotype showed the highest ADG (0.652 ± 0.330 kg/d), whereas cattle with the CC genotype showed the lowest ADG value (0.421 ± 0.178 kg/d).     

胚胎附植期GRB7基因在绵羊子宫内膜中的mRNA表达

旨在探讨生长因子受体结合蛋白7(growth factor receptor bound 7,GRB7)在绵羊胚胎附植期子宫内膜中m RNA的表达模式。应用半定量RT-PCR和实时荧光定量RT-PCR分别检测21 d怀孕母羊全身组织和妊娠第9、13、17、21及25天的怀孕与未孕母羊子宫内膜组织GRB7基因的表达。半定量RT-PCR结果显示,GRB7基因在心脏、皱胃、大肠、小肠、瘤胃、下丘脑、大脑、小脑等组织均未检测出表达,在脾脏、垂体、肾脏、输卵管、卵巢、膀胱及子宫体等组织出现表达,其中在子宫体、输卵管及肾脏中呈现较高表达;实时荧光定量PCR结果显示,从绵羊妊娠第9-25天阶段,GRB7基因在母羊子宫内膜组织的表达量呈逐渐上升趋势,孕羊GRB7的表达量均显著高于同一时间点同期发情的未孕母羊。结果表明GRB7的m RNA表达具有组织特异性,在胚胎附植期绵羊子宫内膜中的m RNA表达显著升高,表明GRB7可能在早期胚胎附植中发挥一定作用。     

牛RHOQ基因的电子克隆与生物信息学分析

利用电子克隆技术获得牛RHOQ基因cDNA序列,采用生物信息学方法对该基因及其编码蛋白的基本理化性质、疏水性、信号肽、二级结构和亚细胞定位等方面进行预测和分析。结果表明,牛RHOQ基因的cDNA序列全长1 517 bp,包含1个618 bp开放阅读框,编码205个氨基酸;其编码蛋白属疏水性蛋白,不存在信号肽及跨膜结构,定位于分泌系统囊泡;二级结构主要以无规则卷曲和α-螺旋为主。牛RHOQ基因编码蛋白可能具有生长因子功能,可能在神经再生和突触延伸过程中起重要作用。     

原因不明子宫内膜薄雌激素受体α基因多态性及其表达

旨在探讨原因不明子宫内膜薄雌激素受体α(estrogen receptor alpha,ERα)基因多态性及其与表达的关系。选择120名原因不明子宫内膜薄患者为试验组,120名子宫内膜正常人群作为对照组。应用分子生物学的方法分析ERα基因PvuⅡ,XbaⅠ限制性片段长度多态性。通过逆转录-多聚酶链反应(RT-PCR)和Western印迹法分析ERα表达。结果显示,P基因型频率试验组为47.1%,对照组为30.0%,OR值:2.076。试验组X基因型频率为20.8%,对照组为30.4%,OR值:0.602。Pvu II和Xba I限制性片段长度多态性在两组中均呈多态性分布。试验组ERα的mRNA和蛋白质表达均比对照组降低(P0.05)。由此得出,ERα基因多态性与原因不明子宫内膜薄有关,P等位基因可能是其危险因素,X等位基因可能是其保护因素。ERα在子宫内膜中原因不明子宫内膜薄中的表达低于子宫内膜厚度正常子宫内膜。